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Quantitative three-dimensional evaluation of immunofluorescence staining for large whole mount spheroids with light sheet microscopy

机译:大型整装球体的免疫荧光染色的三维三维评估采用光片显微镜

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摘要

Three-dimensional cell biology and histology of tissue sections strongly benefit from advanced light microscopy and optimized staining procedures to gather the full three-dimensional information. In particular, the combination of optical clearing with light sheet-based fluorescence microscopy simplifies fast high-quality imaging of thick biological specimens. However, verified in toto immunostaining protocols for large multicellular spheroids or for tissue sections have not been published. We present a method for the verification of immunostaining in three-dimensional spheroids. The analysis relies on three criteria to evaluate the immunostaining quality: quality of the antibody stain specificity, signal intensity achieved by the staining procedure and the correlation of the signal intensity with that of a homogeneously dispersed fluorescent dye. We optimized and investigated variations of five immunostaining protocols for three-dimensional cell biology. Our method is an important contribution to three-dimensional cell biology and the histology of tissues since it allows to evaluate the efficiency of immunostaining protocols for large three-dimensional specimens, and to study the distribution of protein expression and cell types within spheroids and spheroid-specific morphological structures without the need of physical sectioning.
机译:三维细胞生物学和组织切片的组织学极大地受益于先进的光学显微镜和优化的染色程序以收集完整的三维信息。尤其是,将光学清除技术与基于光片的荧光显微镜相结合,可简化厚生物样本的快速高质量成像。但是,尚未针对大型多细胞球体或组织切片的免疫染色方案进行验证。我们提出了一种方法来验证三维球体中的免疫染色。该分析基于三个标准来评估免疫染色质量:抗体染色特异性的质量,通过染色程序获得的信号强度以及信号强度与均匀分散的荧光染料的相关性。我们针对三维细胞生物学优化并研究了五种免疫染色方案的变异。我们的方法为三维细胞生物学和组织组织学做出了重要贡献,因为它可以评估大型三维标本的免疫染色方案的效率,并研究球体和球体中蛋白质表达和细胞类型的分布不需要物理切片的特定形态结构。

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